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Dynamic Switching Mechanisms in LOV1 and LOV2 Domains of Plant Phototropins

机译:植物光蛋白LOV1和LOV2域的动态转换机制

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摘要

LOV domains are the light-sensitive portion of plant phototropins. They absorb light through a flavin cofactor, photochemically form a covalent bond between the chromophore and a cysteine residue in the protein, and proceed to mediate activation of an attached kinase domain. Although the photoreaction itself is now well-characterized experimentally and computationally, it is still unclear how the formation of the adduct leads to kinase activation. We have performed molecular dynamics simulations on the LOV1 domain of Chlamydomonas reinhardtii and the LOV2 domain of Avena sativa, both before and after the photoreaction, to answer this question. The extensive simulations, over 240 ns in duration, reveal significant differences in how the LOV1 and LOV2 domains respond to photoactivation. The simulations indicate that LOV1 activation is likely caused by a change in hydrogen bonding between protein and ligand that destabilizes a highly conserved salt bridge, whereas LOV2 activation seems to result from a change in the flexibility of a set of protein loops. Results of electrostatics calculations, principal component analysis, sequence alignments, and root mean-square deviation analysis corroborate the above findings.
机译:LOV域是植物光蛋白的光敏部分。它们通过黄素辅因子吸收光,以光化学方式在发色团和蛋白质中的半胱氨酸残基之间形成共价键,并继续介导附着的激酶结构域的活化。尽管现在已经通过实验和计算对光反应本身进行了很好的表征,但仍不清楚加合物的形成如何导致激酶活化。在光反应之前和之后,我们已经对莱茵衣藻的LOV1结构域和燕麦Avena的LOV2结构域进行了分子动力学模拟,以回答这个问题。持续时间超过240 ns的广泛仿真显示,LOV1和LOV2域对光激活的反应方式存在显着差异。模拟表明,LOV1激活很可能是由于蛋白质与配体之间的氢键改变而导致高度保守的盐桥不稳定,而LOV2激活似乎是由一组蛋白质环的柔性变化引起的。静电计算,主成分分析,序列比对和均方根偏差分析的结果证实了以上发现。

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